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对编码烟草花叶病毒30千道尔顿蛋白基因的克隆cDNA进行体外转录和翻译。

In vitro transcription and translation of cloned cDNAs encoding the 30-kDa protein gene of TMV.

作者信息

Oliver M J, Deom C M, De B K, Beachy R N

出版信息

Virology. 1986 Nov;155(1):277-83. doi: 10.1016/0042-6822(86)90189-3.

Abstract

A cDNA clone encoding the nonstructural, 30-kDa protein of the common (U1) strain of tobacco mosaic virus (TMV) was isolated and characterized. cDNA clones representing the intact gene as well as deletions from the 5' end of the gene were subcloned into SP6 vectors. Capped RNAs produced by in vitro transcription reactions were translated in a wheat germ cell-free system. The resultant proteins were compared to proteins obtained from the in vitro translation of intermediate length (I2) rods of TMV. Transcripts of the cDNA clones encoded polypeptides of 30, 28, or 18 kDa that were immunoprecipitated by antibody prepared against a synthetic peptide representing the carboxy terminus of the 30-kDa protein. cDNA clones containing the intact 30-kDa sequence coded for 30-kDa polypeptides while clones lacking the 30-kDa initiation codon produced 28-kDa polypeptides. Surprisingly, translation of a transcript from a cDNA clone containing the 30-kDa gene plus 390 nucleotides 5' of the initiator AUG yielded a polypeptide with an approximate molecular mass of 18 kDa. The results indicate that an intact and functional 30-kDa protein gene has been cloned. The significance of these results, with respect to determining the function of the 30-kDa protein, is discussed.

摘要

分离并鉴定了一个编码烟草花叶病毒(TMV)普通(U1)株系非结构30 kDa蛋白的cDNA克隆。将代表完整基因以及基因5'端缺失片段的cDNA克隆亚克隆到SP6载体中。体外转录反应产生的带帽RNA在小麦胚无细胞体系中进行翻译。将所得蛋白质与从TMV中间长度(I2)杆状颗粒的体外翻译获得的蛋白质进行比较。cDNA克隆的转录本编码30 kDa、28 kDa或18 kDa的多肽,这些多肽可被针对代表30 kDa蛋白羧基末端的合成肽制备的抗体免疫沉淀。包含完整30 kDa序列的cDNA克隆编码30 kDa多肽,而缺少30 kDa起始密码子的克隆产生28 kDa多肽。令人惊讶的是,从包含30 kDa基因加上起始AUG上游390个核苷酸的cDNA克隆转录本翻译产生了一种分子量约为18 kDa的多肽。结果表明已克隆到一个完整且有功能的30 kDa蛋白基因。讨论了这些结果对于确定30 kDa蛋白功能的意义。

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